Tissue-derived mesenchymal stromal cells used as vehicles for anti-tumor therapy exert different in vivo effects on migration capacity and tumor growth
Publisher
BioMed CentralDate
2013Citation
10.1186/1741-7015-11-139
BMC Medicine 11.139 (2013): 1-16
ISSN
1741-7015DOI
10.1186/1741-7015-11-139Funded by
This work was supported by FIS (PI080750), DGA (PI041/08, B84, PI086/09), MMA Fund (ICS/08/0050), PROMETEO/2008/163; CTQ-2010-20960-C02-02; S2010/BMD-2349, PIPAMER-0912, and PIPAMER-1214. CB-L was funded by fellowships ICS/08/0050 and DGA PI-086/09, GM by PIPAMER-0912, and PMD by the Araid Fund. We are grateful to Dr Hugo Cabedo and Dr Jose Antonio Gómez-Sánchez for help with the qPCR studies, and to Juan Miguel Sanchez, Camino Latorre, and Rebeca Guerrero for technical assistance. We also thank Professor James McCue and Dr Nancy d’Cruz for their assistance in language editing.Project
Comunidad de Madrid. S2010/BMD-2349/I2M2Editor's Version
http://dx.doi.org/10.1186/1741-7015-11-139; http://www.biomedcentral.com/1741-7015/11/139Subjects
Mesenchymal stromal cells; Migration; In vivo imaging; Tumor growth; Pluripotency; Biología y Biomedicina / BiologíaRights
© 2013 Belmar-Lopez et al.Abstract
Background: Mesenchymal stem cells (MSCs) have been promoted as an attractive option to use as cellular
delivery vehicles to carry anti-tumor agents, owing to their ability to home into tumor sites and secrete cytokines.
Multiple isolated populations have been described as MSCs, but despite extensive in vitro characterization, little is
known about their in vivo behavior.
The aim of this study was to investigate the efficacy and efficiency of different MSC lineages derived from five
different sources (bone marrow, adipose tissue, epithelial endometrium, stroma endometrium, and amniotic
membrane), in order to assess their adequacy for cell-based anti-tumor therapies. Our study shows the crucial
importance of understanding the interaction between MSCs and tumor cells, and provides both information and a
methodological approach, which could be used to develop safer and more accurate targeted therapeutic
applications.
Methods: We first measured the in vivo migration capacity and effect on tumor growth of the different MSCs using
two imaging techniques: (i) single-photon emission computed tomography combined with computed tomography
(SPECT-CT), using the human sodium iodine symporter gene (hNIS) and (ii) magnetic resonance imaging using
superparamagnetic iron oxide. We then sought correlations between these parameters and expression of
pluripotency-related or migration-related genes.
Results: Our results show that migration of human bone marrow-derived MSCs was significantly reduced and
slower than that obtained with the other MSCs assayed and also with human induced pluripotent stem cells
(hiPSCs). The qPCR data clearly show that MSCs and hiPSCs exert a very different pluripotency pattern, which
correlates with the differences observed in their engraftment capacity and with their effects on tumor growth.
Conclusion: This study reveals differences in MSC recruitment/migration toward the tumor site and the
corresponding effects on tumor growth. Three observations stand out: 1) tracking of the stem cell is essential to
check the safety and efficacy of cell therapies; 2) the MSC lineage to be used in the cell therapy needs to be
carefully chosen to balance efficacy and safety for a particular tumor type; and 3) different pluripotency and
mobility patterns can be linked to the engraftment
Files in this item
Google Scholar:Belmar-López, Carolina
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Mendoza, Gracia
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Oberg, Daniel
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Burnet, Jerome
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Simón, Carlos
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Cervello, Irene
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Iglesias, Maite
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Ramírez, Juan Carlos
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López-Larrubia, Pilar
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Quintanilla, Miguel
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Martin-Duque, Pilar
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