AI Article Synopsis

  • The study tests the effectiveness of a novel contrast agent, Gadofluorine M-Cy3 (GdFM-Cy3), for labeling and detecting cardiovascular progenitor cells derived from murine embryonic stem cells (ES-CPC) using cardiac magnetic resonance imaging (CMR).
  • Previous challenges in cell therapy for cardiovascular diseases include accurately identifying transplanted cells, which GdFM-Cy3 aims to address by being easily taken up by cells and allowing for visual detection via CMR.
  • The results showed that GdFM-Cy3 is non-toxic, can be effectively visualized, and successfully identified transplanted ES-CPC in the hearts of mice, confirming its potential utility in improving cell therapy for heart conditions.

Article Abstract

Objectives: The aim of the current study is to test the ability to label and detect murine embryonic stem cell-derived cardiovascular progenitor cells (ES-CPC) with cardiac magnetic resonance (CMR) using the novel contrast agent Gadofluorine M-Cy3 (GdFM-Cy3).

Background: Cell therapy shows great promise for the treatment of cardiovascular disease. An important limitation to previous clinical studies is the inability to accurately identify transplanted cells. GdFM-Cy3 is a lipophilic paramagnetic contrast agent that contains a perfluorinated side chain and an amphiphilic character that allows for micelle formation in an aqueous solution. Previous studies reported that it is easily taken up and stored within the cytosol of mesenchymal stem cells, thereby allowing for paramagnetic cell labeling. Investigators in our laboratory have recently developed techniques for the robust generation of ES-CPC. We reasoned that GdFM-Cy3 would be a promising agent for the in vivo detection of these cells after cardiac cell transplantation.

Methods: ES-CPC were labeled with GdFM-Cy3 by incubation. In vitro studies were performed to assess the impact of GdFM-Cy3 on cell function and survival. A total of 500,000 GdFM-Cy3-labeled ES-CPC or control ES-CPC were injected into the myocardium of mice with and without myocardial infarction. Mice were imaged (9.4-T) before and over a 2-week time interval after stem cell transplantation. Mice were then euthanized, and their hearts were sectioned for fluorescence microscopy.

Results: In vitro studies demonstrated that GdFM-Cy3 was easily transfectable, nontoxic, stayed within cells after labeling, and could be visualized using CMR and fluorescence microscopy. In vivo studies confirmed the efficacy of the agent for the detection of cells transplanted into the hearts of mice after myocardial infarction. A correspondence between CMR and histology was observed.

Conclusions: The results of the current study suggest that it is possible to identify and potentially track GdFM-Cy3-labeled ES-CPC in murine infarct models via CMR.

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Source
http://www.ncbi.nlm.nih.gov/pmc/articles/PMC3638738PMC
http://dx.doi.org/10.1016/j.jcmg.2009.04.015DOI Listing

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