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Abstract #3174

Longitudinal MRI Tracking of Transplanted Neural Progenitor Cells in the Spinal Cord Utilizing the Bright Ferritin Mechanism

Keyu Zhuang1,2, Zixiang Luo3,4,5, Seong Jun Kim3,5, Kyle D.W. Vollett1,2, Hai-Ying Mary Cheng6,7, Mohamad Khazaei3, Michael G. Fehlings3,5,8, and Hai-Ling Margaret Cheng 1,2,9
1Institute of Biomedical Engineering, University of Toronto, Toronto, ON, Canada, 2Translational Biology & Engineering Program, Ted Rogers Centre for Heart Research, Toronto, ON, Canada, 3Division of Genetics and Development, Krembil Research Institute, University Health Network, Toronto, ON, Canada, 4Department of Spine Surgery and Orthopaedics, Xiangya Hospital, Central South University, Changsha, China, 5Institute of Medical Sciences, University of Toronto, Toronto, ON, Canada, 6Department of Biology, University of Toronto Mississauga, Toronto, ON, Canada, 7Department of Cell and Systems Biology, University of Toronto, Toronto, ON, Canada, 8Department of Surgery and Spine Program, University of Toronto, Toronto, ON, Canada, 9The Edward S. Rogers Sr. Department of Electrical and Computer Engineering, University of Toronto, Toronto, ON, Canada

Synopsis

Keywords: Molecular Imaging, Cell Tracking & Reporter Genes

Motivation: A non-invasive imaging technology for monitoring cell survival and in-vivo migration after transplantation is critical to optimizing and translating stem cell-based therapies.

Goal(s): To extend our previously reported bright-ferritin cell tracking platform to monitoring stem cell therapy, we investigated tracking human neural progenitor cells transplanted in the rat spinal cord.

Approach: In-vitro assays of proliferation and differentiation, and imaging both in vitro on cell pellets and in vivo in rats were performed.

Results: Monitoring rats on MRI over seven weeks confirmed the ability to assess cell retention and distribution in the rat spinal cord.

Impact: Our bright-ferritin platform demonstrated no adverse effects on human neural progenitor cells. Stem cells injected in the rat spinal cord could be tracked longitudinally and on-demand via a bright T1-contrast on MRI.

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